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开发用于正常二倍体细胞克隆生长的改良培养基和培养条件。

Development of improved media and culture conditions for clonal growth of normal diploid cells.

作者信息

Ham R G, McKeehan W L

出版信息

In Vitro. 1978 Jan;14(1):11-22. doi: 10.1007/BF02618170.

Abstract

Multiplication of normal diploid cells in culture is controlled by a complex set of interacting extracellular variables. The amount of serum protein needed for colony formation by such cells is affected directly by many of the other variables, including the nature of the culture surface, the type of trypsinization procedure used, and the qualitative and quantitative composition of the culture medium. By a sequential process of adjusting all of these variables to optimum values for cellular multiplication with minimal amounts of serum protein, we have been able to obtain clonal growth of normal human and chicken cells with less than 500 microgram per ml dialyzed serum protein. Precise quantitative adjustment of nutrient concentrations is particularly important. The multiplication-promoting functions of serum can be classified operationally as "replaceable" (those that can be replaced by modifying the medium or the culture conditions) and "nonreplaceable" (those that we have not yet been able to replace). Elimination of the requirement for replaceable functions of serum has improved greatly the specificity and sensitivity of the bioassay for the nonreplaceable functions. The nonreplaceable multiplication-promoting activity from fetal bovine serum for human diploid fibroblasts has been separated from fetuin and serum albumin and purified approximately 15-fold.

摘要

培养中正常二倍体细胞的增殖受一系列复杂的细胞外相互作用变量控制。此类细胞形成集落所需的血清蛋白量直接受许多其他变量影响,包括培养表面的性质、所用胰蛋白酶消化程序的类型以及培养基的定性和定量组成。通过将所有这些变量依次调整到细胞增殖的最佳值,同时使用最少的血清蛋白,我们已能够在每毫升透析血清蛋白低于500微克的情况下实现正常人细胞和鸡细胞的克隆生长。精确的营养物浓度定量调整尤为重要。血清的增殖促进功能可在操作上分为“可替代的”(那些可通过改变培养基或培养条件来替代的功能)和“不可替代的”(那些我们尚未能够替代的功能)。消除对血清可替代功能的需求极大地提高了对不可替代功能生物测定的特异性和灵敏度。来自胎牛血清的对人二倍体成纤维细胞不可替代的增殖促进活性已从胎球蛋白和血清白蛋白中分离出来,并纯化了约15倍。

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